toxico studiu 2
TRANSCRIPT
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Glucocorticoids Alter Craniofacial Development and Increase Expression and Activity of
Matrix Metalloproteinases in Developing Zebrafish (Danio rerio)
Jedd M. Hillegass, Caren M. Villano, Keith R. Cooper and Lori A. White1
Author Affiliations
Joint Graduate Program in Toxicology, Rutgers, The State University of New Jersey, New
Brunswick, New Jersey 08901
Abstract
Teratogenic effects are observed following long-term administration of glucocorticoids,
although short-term glucocorticoid therapy is still utilized to reduce fetal mortality, respiratory
distress syndrome, and intraventricular hemorrhage in preterm infants. However, the mechanism of
glucocorticoid-induced teratogenicity is unknown. We hypothesize that glucocorticoid-induced
teratogenesis is mediated through the glucocorticoid receptor (GR) and results from altering theexpression and activity of the matrix metalloproteinases (MMPs). During embryogenesis,
degradation of the extracellular matrix to allow for proper cellular migration and tissue
organization is a tightly regulated process requiring appropriate temporal and spatial expression
and activity of the MMPs. Studies have demonstrated that MMP gene expression can be either
inhibited or induced by glucocorticoids in a variety of model systems. Using the zebrafish (Danio
rerio) as a model of development, the data presented here demonstrate that embryonic exposure to
the glucocorticoids dexamethasone or hydrocortisone increased expression of two gelatinases,
MMP-2 (1.5-fold) and MMP-9 (7.6- to 9.0-fold), at 72 h postfertilization (hpf). Further,
gelatinase activity was increased approximately threefold at 72 hpf following glucocorticoid
treatment, and changes in craniofacial morphogenesis were also observed. Cotreatment of
zebrafish embryos with each glucocorticoid and the GR antagonist RU486 resulted in attenuation
of glucocorticoid-induced increases in MMP expression (5284% decrease) and activity (4194%
decrease). Furthermore, the abnormal craniofacial phenotype observed following glucocorticoid
exposure was less severe following RU486 cotreatment. These studies demonstrate that in the
embryonic zebrafish, dexamethasone, and hydrocortisone alter expression and activity of MMP-2
and -9, and suggest that these increases may be mediated through the GR.
Glucocorticoids play a central role in vertebrate physiology and are involved in numerous
regulatory mechanisms associated with development, bone replication, bone differentiation,
apoptosis, metabolism, circadian cell cycle rhythmicity, and the stress response, among others
(Canalis and Delany, 2002; Dickmeis et al., 2007). Glucocorticoids act as immunosuppressive and
anti-inflammatory agents, and are therefore widely utilized to treat autoimmune and inflammatory
disorders, transplant rejection, and lymphoproliferative diseases (Almawi et al., 2002). These
compounds are also potent teratogens whose antenatal use has been linked to fetal growth
restriction and cleft palate (Abbott, 1995; Mandl et al., 2006), and intrauterine programming of
metabolic, neuroendocrine and cardiovascular disorders in adult life (Seckl, 2004). The exact
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mechanism by which glucocorticoids exert their teratogenic effects is unknown, although recent
work in the zebrafish has demonstrated that these compounds are capable of upregulating matrix
metalloproteinase-13 (MMP-13) (Hillegass et al., 2007). Further, glucocorticoids have been shown
to stimulate MMP-9 expression through induction of soluble glucocorticoid-induced tumor
necrosis factor receptor in murine macrophages (Lee et al., 2003, 2004). These results sit in direct
opposition to what has been found in mammalian cell models in vitro, where MMP expression is
inhibited by exposure to glucocorticoids (Canalis and Delany, 2002; Chakraborti et al., 2003;
Vincenti et al., 1996). Despite contradictory findings, these studies suggest MMPs may be pivotal
in eliciting glucocorticoid-induced teratogenicity and support further examination of the
mechanism.
Extracellular matrix (ECM) remodeling is essential for a number of physiological
processes including embryonic development, reproduction, tissue resorption, wound healing, and
apoptosis (Brinckerhoff and Matrisian, 2002; Hulboy et al., 1997; Nagase and Woessner, 1999).
Central to these processes are MMPs, a group of over twenty zinc-dependent endopeptidases
responsible for precise and regulated ECM degradation. Dysregulation and excessive expression of
MMPs have been tied to a number of pathological disorders such as osteo- and rheumatoid
arthritis, emphysema, multiple sclerosis, bacterial meningitis, and tumor invasion and metastasis
(D'Armiento et al., 1992; Folgueras et al., 2004; Hendrix et al., 2003; Leppert et al., 2001;
Rundhaug, 2005). Recent work using zebrafish has focused on the role of MMPs during embryonic
development. Our laboratory and others have shown that MMP-2, MMP-9, MMP-13, and
membrane-type MMP- and - are required for normal zebrafish embryogenesis (Hillegass et al.,
2007, unpublished data; Zhang et al., 2003a, b).
Most glucocorticoid-associated effects are mediated through the glucocorticoid receptor
(GR), which belongs to the nuclear receptor superfamily and acts as a ligand-dependent
transcription factor (Evans, 2005). A single GR has been identified in zebrafish thus far, although
other related teleosts have two distinct GR genes (Bury et al., 2003; Greenwood et al., 2003). The
teleost GR is unique from the mammalian GR in that the DNA-binding domain contains nine
additional residues between the two zinc fingers. These nine amino acid inserts are remarkably
conserved among teleostean fish species (Stolte et al., 2006; Terova et al., 2005) and appear to be
the result of alternative splicing (Stolte et al., 2006). It has been suggested that because these
residues promote greater DNA affinity in the GR, they could have been selected to serve the large
spectrum of cortisol functions in fish (Lethimonier et al., 2002). Such GR splice variants have been
characterized in the rainbow trout (Bury et al., 2003) and Burtons' mouthbrooder (Greenwood etal., 2003; Takeo et al., 1996) thus far, and it is believed this could result in separate biological
functions for each receptor variant (Prunet et al., 2006).
The purpose of these studies is to examine the effects of the glucocorticoids
dexamethasone and hydrocortisone on MMP-2 and MMP-9 expression and activity and to
establish a causal link between activation of the GR and changes in MMP-2, MMP-9, and MMP-
13 levels. Further we wish to better characterize the craniofacial defects known to result from
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exposure of embryonic zebrafish to these glucocorticoids. The gelatinases MMP-2 (gelatinase A)
and MMP-9 (gelatinase B) readily degrade gelatins (denatured collagens) and intact collagen type
IV, and the collagenase MMP-13 (collagenase-3) cleaves native interstitial collagens I, II, and III
(Chakraborti et al., 2003). These particular MMPs were selected because they have been shown to
be vital for normal development in both zebrafish and mice (Inada et al., 2004; Itoh et al., 1997;
Mosig et al., 2007; Stickens et al., 2004; Vu et al., 1998). The data presented in this paper
demonstrate that dexamethasone and hydrocortisone cause increases in MMP-2 and MMP-9
expression and activity in the zebrafish embryo at 72 h postfertilization (hpf), with resultant
changes in craniofacial morphogenesis. Cotreatment with glucocorticoids and the GR antagonist
RU486 results in attenuation of the increases in MMP-2, MMP-9, and MMP-13 expression and
activity normally observed following glucocorticoid treatment, as well as a partial rescue of the
abnormal craniofacial phenotype. These results further demonstrate that in the embryonic
zebrafish, dexamethasone, and hydrocortisone alter expression and activity of MMPs, including
MMP-2 and -9, and suggest that these increases may be mediated through the GR.
MATERIALS AND METHODS
Zebrafish strains and husbandry.
The AB strain of zebrafish (Danio rerio), obtained from the Zebrafish International
Resource Center, was used for all of the experiments described. Zebrafish were maintained and
bred in an Aquatic Habitats recirculation system according to a husbandry protocol approved by
the Rutgers University Animal Care and Facilities Committee.
Collection and treatment of zebrafish embryos.
Embryos were collected from breeding stocks of zebrafish and treated starting at 3 hpf.
Treatments consisted of continuous (i.e., without renewal) exposure through 24, 48, 72, or 96 hpf
to 100 mg/l of dexamethasone (254.81M equivalent) or hydrocortisone (275.88M equivalent)
alone or in conjunction with 100250nM mifepristone (RU486) in embryo medium (Westerfield,
2000). This dose of dexamethasone or hydrocortisone has been shown in our laboratory to be
effective in inducing MMP-13 levels in developing zebrafish (Hillegass et al., 2007).
Dexamethasone and hydrocortisone were dissolved in dimethylformamide (DMF) prior to being
diluted in embryo medium to the experimental concentrations. In order to generate experimental
concentrations of RU486, a 1mM stock of RU486 was first made by dissolving in 100% ethanol,
and a subsequent 100M working stock was generated by further dilution into ethanol. Finalconcentrations of RU486 were achieved by diluting this working stock in embryo medium. All
RU486 stocks were stored at 20C between uses. Controls, including a no treatment control of
embryo medium alone and a solvent control consisting of ethanol and/or DMF alone were run
concurrently with each treatment. When cotreatments of dexamethasone or hydrocortisone and
RU486 were performed, a RU486 control consisting of the appropriate concentration of RU486
alone was included. The no treatment control embryos were monitored throughout the course of
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each study to confirm embryo viability. Data from any treatment in which > 10% of the solvent or
no treatment control embryos exhibited developmental abnormalities were not considered for
analysis. All chemicals and solvents were purchased from Sigma-Aldrich (St Louis, MO) and
possessed purities 98%.
Real-time reverse transcriptionPCR.
Embryos collected for RNA isolation (n = 50100) were snap frozen in 1.5-ml
microcentrifuge tubes using liquid nitrogen and stored at 80C. Total RNA was isolated from
embryos using TRIzol (Invitrogen Carlsbad, CA) and DNase-treated (DNA-free kit, Ambion
Austin, TX) to remove genomic DNA contamination. Total RNA yields were typically 12 g/l.
Reverse transcription was performed on 1 g aliquots of total RNA to produce complimentary
DNA (cDNA) for real-time reverse transcriptionPCR (RT-PCR) (quantitative RT-PCR; qRT-
PCR) using an iScript cDNA Synthesis Kit (BioRad Hercules, CA). Real-time RT-PCR reactions
were performed in triplicate using BioRad iQ SYBR Green Supermix, and cDNA amplification
was performed for 40 cycles on a BioRad iCycler equipped with an iCycler iQ Detection System.Primers to zebrafish -actin, MMP-2, MMP-9, and MMP-13 were used in amplification reactions.
For -actin, the forward primer was 5-CGAGCAGGAGATGGGAACC-3 and the reverse primer
was 5-CAACGGAAACGCTCATTGC-3 giving a product size of 102 base pairs (bp). For MMP-
2, the forward primer was 5-AGCTTTGACGATGACCGCAAATGG -3 and the reverse primer
was 5-GCCAATGGCTTGTCTGTTGGTTCT-3 giving a product size of 224 bp. For MMP-9, the
forward primer was 5-AACCACCGCAGACTATGACAAGGA-3 and the reverse primer was 5-
GTGCTTCATTGCTGTTCCCGTCAA-3 giving a product size of 89 bp. For MMP-13, the
forward primer was 5-ATGGTGCAAGGCTATCCCAAGAGT-3 and the reverse primer was 5-
GCCTGTTGTTGGAGCCAAACTCAA-3 giving a product size of 289 bp. Real-time threshold
cycle data were normalized to -actin, which served as a loading control, and standard curves
generated for MMP-2, MMP-9, and MMP-13 were used to quantify messenger RNA (mRNA)
expression.
In situ hybridization.
The MMP-2 RNA probe was generated using a construct generously donated by Dr Robert
Tanguay (Oregon State University) consisting of full-length MMP-2 cDNA expressed in pCR-
Blunt II-TOPO. The plasmid was linearized using PstI, and SP6 and T7 RNA polymerase were
used to generate antisense and sense, respectively, digoxigenin (DIG)-labeled RNA probes (DIG
RNA Labeling Kit-SP6/T7, Roche Indianapolis, IN). The MMP-9 RNA probe was generated froma cDNA clone encoding a 318-bp portion of the MMP-9 gene amplified using the following
primers: 5-TTTGAGCTCTACAGTCTGTTTCTGGTGG-3 (forward primer; the italicized portion
designates a SacI restriction site) and 5-ATAGGATCCGGCGTCAAACTCCTT-3 (reverse
primer; the italicized portion designates a BamHI restriction site). To generate this portion of the
MMP-9 gene, total RNA from untreated 72 hpf embryos was isolated, DNase-treated, made into
cDNA as described previously and polymerase-amplified via PCR. The 318-bp PCR product was
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digested using SacI and BamHI restriction enzymes and subsequently cloned into PSPT18
(Roche). The PSPT18-MMP9 construct was linearized with BamHI, and SP6 and T7 RNA
polymerase were used to create sense and antisense probes, respectively.
Embryos to be used for in situ hybridization were grown in 0.003% (0.033 mg/ml in
embryo medium) phenylthiourea (Sigma) to inhibit formation of pigmentation. Prior to initiationof staining, embryos were dechorionated, euthanatized using an overdose of MS-222 (Sigma), and
fixed overnight in BT-fix (4% sucrose, 4% paraformaldehyde, 0.1M sodium phosphate, 0.15mM
calcium chloride, titrated to pH 7.3) (Westerfield, 2000). The in situ hybridization protocol
followed was a slight modification of that described by (Oxtoby and Jowett, 1993). Following
staining, the embryos were cleared of nonspecific staining by being transferred into methanol for
10 min, soaked in isopropanol for 10 min, and then placed in 1,2,3,4-tetrahydronaphthalene
(Sigma-Aldrich) for visualization.
In vitro zymography.
Lysates were prepared from 72 hpf zebrafish embryos (n = 3050) as described by
(Crawford and Pilgrim, 2005). Lysate protein concentration was determined using a Modified
Lowry Protein Assay Kit (Pierce Rockford, IL) to ensure that each reaction contained equal
amounts of total protein. In vitro zymography reactions were set up in 96-well plates as follows: 1
l of lysate (corresponding to approximately 0.214 g total protein), 10 l of 1 mg/ml
fluoresceinated type I or type IV DQ Collagen (Molecular Probes Carlsbad, CA), and lysis buffer
(150mM NaCl, 10mM 4-(2-hydroxyethyl)-1-piperazineethanesulfonic acid, 2mM dithiotreitol,
0.1% Triton X-100, pH 8.0) to bring the volume to 200 l. Ethylenediaminetetraacetic acid
(EDTA) (1mM), GM6001 (100M; Calbiochem Gibbstown, NJ), and MMP-2/MMP-9 inhibitor II
(100M; Calbiochem; Tamura et al., 1998) were added to these reactions as inhibitors. Wheninhibitors were utilized, reactions consisting of lysate, lysis buffer, and inhibitor only were allowed
to preincubate overnight prior to addition of fluoresceinated substrate. Following preincubation,
reactions were incubated for 24-72 h prior to measurement. Fluorescein isothiocyanate
fluorescence was measured using a Perkin Elmer (Waltham, MA) HTS 7000 Plus Bio Assay
Reader set for excitation at 492 nm and emission detection at 535 nm. All reactions were run in at
least triplicate and were corrected for background fluorescence.
Alcian blue staining.
Embryos to be used for Alcian blue staining were grown in 0.003% phenylthiourea.Embryos were euthanatized using an overdose of MS-222, fixed overnight at 4C in 4%
paraformaldehyde, and then transferred to 70% ethanol to allow dehydration of the tissue for at
least 24 h. Prior to staining, embryos were bleached in 30% hydrogen peroxide for approximately
2 h and then rinsed twice with 0.1% Tween-20 in phosphate buffered saline. Staining was
performed overnight at room temperature using 0.1% Alcian blue 8GX (Sigma-Aldrich) that had
been filtered through a 2 m syringe filter. Following staining, embryos were placed in acidified
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ethanol for 24 h to allow for clearing of nonspecific staining. Finally embryos were washed in
increasing concentrations of glycerol (15 min each of 20%, 50%, 80%, and 100%) and visualized
as described previously.
Statistical analysis.
Statistical analysis was performed using the SigmaStat v1.0 computer software package
(Jandel Scientific San Rafael, CA). Data were evaluated by one-way analysis of variance
(ANOVA), and Dunnett's test or the Bonferroni t-test was used as the multiple comparison method.
The probability level for statistical significance was p < 0.05.
RESULTS
Exposure to Dexamethasone or Hydrocortisone Causes an Induction of MMP-2 and MMP-
9 mRNA in Zebrafish Embryos
Previous studies from our laboratory show that zebrafish embryos respond todexamethasone and hydrocortisone in a dose-dependent manner, and that a dose of 100 mg/l is
required to generate responses in both MMP-13 mRNA expression level and phenotype (Hillegass
et al., 2007). Embryos exposed to 100 mg/l dexamethasone or hydrocortisone demonstrate a
significant (p < 0.05) increase in MMP-2 and MMP-9 mRNA at 72 hpf measured via qRT-PCR
(Fig. 1). Dexamethasone- and hydrocortisone-treated embryos exhibit a 1.6- and 1.5-fold induction
in MMP-2 mRNA over solvent-control treated embryos, respectively. A 9.0- and 7.6-fold
induction in MMP-9 mRNA is also observed in dexamethasone- and hydrocortisone-treated
embryos, respectively. In situ hybridization of 72 hpf embryos using either a MMP-2specific or
MMP-9specific mRNA probe confirms the glucocorticoid-induced increase in expression
observed via qRT-PCR (Fig. 2). Sense probes for each of these MMPs yield essentially no signal
and confirm the specificity of the antisense probes (data not shown). For MMP-2, solvent control
embryos express transcript throughout their entire body, with the exception of the yolk sac and
yolk sac extension. Slightly higher levels of MMP-2 expression appear to be localized rostrally and
distinct areas of expression are observed in the neurocranial cartilage, midbrain, heart, and anterior
kidney. Following treatment with either dexamethasone or hydrocortisone, increased transcript
levels are seen in both the medial and lateral aspects of the trunk, the anterior kidney, the heart, and
several areas associated with the head specifically. These include the neurocranial cartilage,
pharyngeal cartilage, and midbrain. MMP-9 transcript in solvent control embryos is also localized
rostrally, although some expression is seen in medial trunk superior to the yolk sac extension.Glucocorticoid-treated embryos exhibit increased MMP-9 expression levels throughout their entire
trunk and head. Given the intensity of signal present in the embryo head following treatment with
dexamethasone or hydrocortisone, it is difficult to distinguish explicit areas of increased
expression.
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FIG. 1. qRT-PCR reveals that MMP-2 and MMP-9 mRNA expression is increased in zebrafish
embryos at 72 hpf following exposure to 100 mg/l dexamethasone or hydrocortisone. Zebrafish
embryos (n = 50100) were continuously exposed to treatments starting at 3 hpf for 24, 48, or 72
hours, and total RNA was isolated for use as template in qRT-PCR. Typical RNA yields were 12
g/l and 1 g aliquots of this RNA were used to produce template cDNA. Data were quantified byutilizing standard curves generated from specific PCR products at concentrations ranging from 1
ng to 500 fg. Data were normalized to -actin. PCR reactions were performed in triplicate and
data are representative of three separate experiments. Error bars denote standard deviation. A
statistically significant increase in (A) MMP-2 and (B) MMP-9 expression in glucocorticoid-
treated embryos is observed at 72 hpf as determined via one-way ANOVA and Dunnett's test (*p